ProcartaPlex™ Human Th1/Th2 Cytokine Panel, 11plex

Citations & References (7)

Invitrogen™

ProcartaPlex™ Human Th1/Th2 Cytokine Panel, 11plex

製品番号（カタログ番号）	数量
EPX110-10810-901	96テスト

製品番号（カタログ番号） EPX110-10810-901

価格（JPY）

455,300

お問い合わせください ›

96テスト

Th1/Th2ケモカイン11-プレックスヒトProcartaPlexパネルは、Luminex xMAP技術を使用して1つのウェルで11のタンパク質ターゲットを分析することにより、Th1/Th2応答の研究を可能にします。このパネルは、サイトカイン／ケモカイン／増殖因子45-Plex ProcartaPlexパネル1のモジュールです（カタログ番号EPX450-12171-901）。このキットは、45プレックスパネルの標的に対応する他のモジュールまたは個別シンプレックスアッセイと完全に組み合わせ可能です。

ProcartaPlex事前設定済みパネルは、検体の組み合わせ性、干渉、交差反応性について広範にテストされており、最高レベルの検証と精度を提供します。すべての ProcartaPlex パネルには、アッセイの実行に必要な試薬が付属しています。

ProcartaPlexマルチプレックスパネルは、6 種の生物種（ヒト、マウス、ラット、ヒト以外の霊長類、ブタ、イヌ）にわたって複数のフォーマットで利用可能です。詳細と利用可能な製品については、ProcartaPlexイムノアッセイページをご覧ください。

ターゲットリスト[ビーズ領域]： GM-CSF [44], IFNγ [43], IL-1β [18], IL-2 [19], IL-4 [20], IL-5 [21], IL-6 [25], IL-12p70 [34], IL-13 [35], IL-18 [66], TNFα [45]

Luminexプラットフォーム用ProcartaPlexアッセイについて
ProcartaPlexイムノアッセイはサンドイッチELISAの原理に基づいており、1つのタンパク質の異なるエピトープに結合する2つの高特異性抗体を使用して、Luminex装置により、すべてのタンパク質ターゲットを同時に定量できます。ProcartaPlexマルチプレックスアッセイは、25 µLの血漿または血清、または50 µLの細胞培養上清のみが必要で、わずか4時間で分析結果が得られます。

次の特長があります。
• 再現性と信頼性の高い結果—タンパク質標的の結合性や交差反応性試験など、業界最高水準のパネルとして検証済み
• サンプルあたりの結果の増加—25～50 µLのサンプル1つで複数のタンパク質標的を同時に測定
• 定評のあるLuminex技術高参照マルチプレックスプラットフォームによるタンパク質の検出および定量

ProcartaPlexアッセイでは、Luminex xMAP（多項目同時測定プロファイリング）技術を利用して、25～50 µLのサンプル1つで最大65のタンパク質標的（血漿、血清、細胞培養上清、およびその他の体液）を同時に検出および定量できます。

ProcartaPlex アッセイの Luminex ビーズは、赤および赤外フルオロフォアの正確な比率で内部染色されており、Luminex xMAP 検出システム（Luminex 200、FLEXMAP 3D、MAGPIX など）により識別できるスペクトル的に固有なシグネチャを生じます。サンドイッチ ELISA と同様に、ProcartaPlex アッセイはマッチした抗体ペアを使用して目的のタンパク質を同定します。マルチプレックスアッセイでは、各スペクトルに固有のビーズは単一の標的タンパク質に特異的な抗体で標識され、結合したタンパク質はビオチン化抗体およびストレプトアビジン-R-フィコエリトリン（ RPE）で同定されます。タンパク質特異的抗体の特異的なビーズへの結合により、1 つのウェルで複数のターゲットの分析が可能になります。

ProcartaPlex アッセイと ELISA の最も大きな違いは、ProcartaPlex アッセイの捕捉抗体がビーズに結合され、マイクロプレートウェルに吸着されないことです。そのため、ProcartaPlex アッセイ試薬は溶液中で自由に浮遊します。たとえば、Luminex 200装置は検出用に2つのレーザーを備えています。1つは各ビーズのスペクトル特性を識別するためのレーザーで、もう1つはサンプル中のタンパク質量に比例したRPE蛍光量を定量するためのレーザーです。ProcartaPlexマルチプレックスアッセイは、従来のサンドウィッチELISAの実行に要する時間で、大幅に少ないサンプル量を使用して、より多くのターゲットタンパク質をプロファイルできます。

ProcartaPlexマルチプレックスパネルは、6種の生物種（ヒト、マウス、ラット、ヒト以外の霊長類、ブタ、イヌ）にわたって複数のフォーマットで利用可能です。詳細および利用可能な製品については、thermofisher.com/procartaplex をご覧ください。

研究用途にのみご使用ください。診断目的には使用できません。

アッセイ範囲分析証明書を参照

アッセイ感度15%未満

使用対象 (装置)Luminex™ 装置

フォーマットMultiplex Kit

製品ラインProcartaPlex

サンプルタイプ血清、血漿、細胞培養上清, Plasma, Cell Culture Supernatants

サンプル量血清、血漿：25 μL、CCS：50 μL

出荷条件湿氷

CombinabilityCombinable

製品タイプマルチプレックスパネル

数量96テスト

Research AreaImmunology, Cytokines

種Human

Unit SizeEach

組成および保存条件

ヒト標準ミックスA（凍結乾燥）バイアル2本
キャプチャービーズミックス（1X）バイアル1本
ビオチン化検出抗体ミックス（50X）バイアル1本
読み取りバッファー（1X）ボトル1本
洗浄バッファー（10X）ボトル1本
ストレプトアビジン-PE（1X）ボトル1本
ユニバーサルアッセイバッファー（1X）ボトル1本
検出抗体希釈液（1X）ボトル1本
8チューブストリップ
接着フィルム
平底96ウェルプレート、黒
2℃～8℃で保存してください

よくあるご質問（FAQ）

What is the size of the Luminex beads you currently use?

The beads used in our Luminex instrument-compatible ProcartaPlex and QuantiGene Plex assays are 6.5 micron superparamagnetic beads.

Find additional tips, troubleshooting help, and resources within our Protein Assays and Analysis Support Center.

I am interested in performing Luminex assays using BioSource kits, and I have a Luminex xMAP system. Besides the kits and system, what other reagents and equipment will I need?

The following is a list of general lab supplies that are required for running BioSource immunoassays on the Luminex xMAP system:
1) Sonicating water bath
2) Orbital shaker
3) Vortexer
4) Repeating and/or multi-channel pipetter (not required, but recommended)
5) Calibrated adjustable precision pipettes, with disposable plastic tips
6) Glass/plastic tubes and racks for preparing reagents
7) Graduated cylinder and container for preparing wash solution
8) Aluminum foil
9) Deionized or distilled water.

Find additional tips, troubleshooting help, and resources within our Protein Assays and Analysis Support Center.

Do the Luminex beads require special care in handling?

The Luminex beads should be protected from light because they are susceptible to photobleaching. We recommend protecting the beads by keeping containers covered with aluminum foil during all incubation steps, and exercising care during handling. The beads should not be frozen, subjected to excessive heat, or exposed to organic solvents.

Find additional tips, troubleshooting help, and resources within our Protein Assays and Analysis Support Center.

Why would the Luminex acquisition software display "Sample Empty" messages during analysis?

(1) The user did not properly aliquot the diluted beads, such that no beads were actually added to the wells (make sure that the bead concentrates are sonicated and vortexed well, then check the pipet tip to ensure that air bubbles were not drawn up)
(2) The user missed loading diluted beads to some wells, which is likely since the small volume is clear and difficult to visualize in the clear plastic plate (we have now addressed this customer difficulty by coloring each of the Buffer Reagent Kit components)
(3) The user applied too much vacuum pressure at some point during the wash steps, or allowed the pressure to spike even once, such that the filter membrane tore in a few wells releasing the beads (make sure that the vacuum manifold pressure is kept below 5mm/in Hg, depending on their system -- a good rule of thumb is that it should take a full 3-second count to GENTLY empty the wells of 200uL)
(4) The user did not properly sonicate and vortex the beads prior to dilution, such that the percent of bead aggregation was high and the instrument was unable to find enough single beads to meet the events/bead value designated by the customer (make sure that the Bead Concentrate tube is put into the waterbath all the way to the cap, since the tube is hollow until the top third)
(5) The user lost beads by shaking the plate too aggressively or handling it improperly (make sure that the orbital shaker is set to a speed that allows for maximum vortex in the wells without spillage)
(6) The user exposed the beads to an excess of light during storage or running of the assay, such that some but not all of the beads were photobleached and therefore falling outside the acceptable range for each bead region (make sure that the plate is covered on the top/sides with foil throughout the assay, away from Windows and spotlights, and that the bead component of the kits is stored in the dark)*
(7) There was a clog in the sample needle, such that the instrument was unable to take up enough sample to meet the number of events requested per bead region (suggest that the user follow the manual instructions for dislodging a clog, which include several Back Flush steps and may require removal of the needle for sonication with probe alignment).

* Some of the older Antibody Bead Kits still have clear plastic tops instead of black ones. In cases where customers store kits in lit refrigerators, or keep them open on the lab bench, even a few hours of light exposure is enough to photobleach beads. It is important to note, in general, that higher number bead regions are more susceptible to photobleaching. In order to draw conclusions about the source of the difficulty, we would ask to see the data, specifically the Masterplex QT file, which would enable us to examine the pattern of "Sample Empty" occurrences in addition to the bead counts per well.

Find additional tips, troubleshooting help, and resources within our Protein Assays and Analysis Support Center.

What are the Luminex beads made of?

The beads are made of polystyrene.

Find additional tips, troubleshooting help, and resources within our Protein Assays and Analysis Support Center.

View all ProcartaPlex™ Human Th1/Th2 Cytokine Panel, 11plex FAQs

引用および参考文献 (7)

引用および参考文献

Abstract

Novel three-dimensional biochip pulmonary sarcoidosis model.

Authors:Calcagno TM, Zhang C, Tian R, Ebrahimi B, Mirsaeidi M

Journal:PLoS One

PubMed ID:33539409

'Sarcoidosis is a multi-system disorder of granulomatous inflammation which most commonly affects the lungs. Its etiology and pathogenesis are not well defined in part due to the lack of reliable modeling. Here, we present the development of an in vitro three-dimensional lung-on-chip biochip designed to mimic granuloma formation. A lung ... More

Serum Cytokines Th1, Th2, and Th17 Expression Profiling in Active Lupus Nephritis-IV: From a Southern Chinese Han Population.

Authors:Sigdel KR, Duan L, Wang Y, Hu W, Wang N, Sun Q, Liu Q, Liu X, Hou X, Cheng A, Shi G, Zhang Y

Journal:Mediators Inflamm

PubMed ID:27738386

'Systemic lupus erythematosus (SLE) is a chronic autoimmune disease characterized by aberrant T cell immune response. Diffuse proliferative lupus nephritis (LN-IV) is the most common, severe, and active form of lupus nephritis. In this study, we investigated the production of Th1, Th2, and Th17 cytokines in prediction of active form ... More

Levels of interleukin (IL)-6 and IL-8 are elevated in serum and bronchoalveolar lavage fluid of haematological patients with invasive pulmonary aspergillosis.

Authors:Heldt S, Eigl S, Prattes J, Flick H, Rabensteiner J, Prüller F, Niedrist T, Neumeister P, Wölfler A, Strohmaier H, Krause R, Hoenigl M

Journal:Mycoses

PubMed ID:28877383

Aspergillus spp. have been shown to induce T-helper cell (Th) 1 and Th17 subsets resulting in elevated levels of several cytokines. The objective of this study was to analyse a bundle of cytokines in serum and bronchoalveolar lavage fluid (BALF) in patients with and without invasive pulmonary aspergillosis (IPA). This ... More

Association between Interleukin-6 Levels and Perioperative Fatigue in Gastric Adenocarcinoma Patients.

Authors:Wu JM, Yang HT, Ho TW, Shun SC, Lin MT

Journal:J Clin Med

PubMed ID:31010015

Gastric adenocarcinoma (GA), one of the most common gastrointestinal cancers worldwide, is often accompanied by cancer cachexia in the advanced stage owing to malnutrition and cancer-related symptoms. Although resection is the most effective curative procedure for GA patients, it may cause perioperative fatigue, worsening the extent of cancer cachexia. Although ... More

Stem Cells from Human Extracted Deciduous Teeth Expanded in Foetal Bovine and Human Sera Express Different Paracrine Factors After Exposure to Freshly Prepared Human Serum.

Authors:Haque N, Widera D, Abu Kasim NH

Journal:Adv Exp Med Biol

PubMed ID:30771186

The response of stem cells to paracrine factors within the host's body plays an important role in the regeneration process after transplantation. The aim of this study was to determine the viability and paracrine factor profile of stem cells from human extracted deciduous teeth (SHED) pre-cultivated in media supplemented with ... More

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